Abstract
We here describe a mutant low density lipoprotein receptor gene that produces a shortened receptor protein lacking three domains: the region of clustered O-linked carbohydrates, the membrane-spanning region, and the cytoplasmic tail. The defect is attributable to a single nucleotide substitution that creates a premature termination codon at amino acid 660, eliminating 180 residues from the mature protein. The truncated protein retains only two domains: a complete ligand-binding region (residues 1-292) and a partial epidermal growth factor precursor homology region (residues 293-659). The termination codon occurs in the middle of a cysteine-rich sequence that is part of the epidermal growth factor precursor homology domain. The mutant protein is present in markedly reduced amounts and may be translated at a reduced rate. After synthesis, most of the receptor remains within the cell for several hours with its N-linked carbohydrate in an unprocessed endoglycosidase H-sensitive form. This finding suggests that the shortened receptor leaves the endoplasmic reticulum at an abnormally slow rate, which is likely attributable to abnormal folding of the truncated protein. The mutation creates a new restriction site for the enzyme HinfI, thus permitting diagnosis by Southern blotting of genomic DNA. Two copies of this mutant gene were present in each of four unrelated Arab patients with homozygous familial hypercholesterolemia (three from Lebanon and one from Syria). We believe that this mutation, hereafter referred to as the "Lebanese allele," is responsible for the extraordinarily high incidence of familial hypercholesterolemia in Lebanon.
Highlights
From the $Departments of Moleculur Geneticsand Internal Medicine, University of Texaa Health Science Center at Dallas, Southwestern Medical School,Dallas, Texas 75235 and t k **Division of Hemtohgy-Oncohgy, Departments of Internal Medicine and Biochemistry, Washington University School of Medicine, St
The familial hypercholesterolemia (FH) 264 cells showed no detectable high affinity After incubation for 48 h in lipoprotein-deficient serum (day 7 of binding, uptake, or degradation of lz5I-LDL.Table I shows that cells from three other individuals from different Arab families (FH 550 and 786 from Lebanon and FH 793 from Syria) show a marked reduction in high affinity binding, cell growth), each monolayer received 2 mlof medium containing 10%lipoprotein-deficient serum and 10 fig of protein/ml of "3-LDL
The data shown represent high affinity values, which and FH 550 failed to bind '251-labeledIgG-C7 at 4 "C, a monoclonal antibody directed against the LDL receptor, indicating that no immunoreactive receptor reached the surface of these cells (Table 11)
Summary
Fibroblasts.After incubation for 48 h inlipoprotein-deficient serum (day 7 of cell growth), each monolayer received 2 ml of medium containing lipoprotein-deficient serum and the indicated concentration of lZ6I-LDL(109 cpm/ng). After incubation for 5 h at 37 "C,the total values for surface-bound, intracellular, and degraded 'T-LDL were determined. The datawere not corrected for nonspecificbinding, uptake, ordegradation of '=I-LDL
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